Sample preparation methods

ABSTRACT

The present invention provides whole blood nucleic acid extraction methods, compositions, and kits, as well as nested isothermal amplification methods, compositions, and kits. In certain embodiments, these methods are applied to detecting Lyme disease, including in patients without classic erythema migrans skin lesions.

CROSS-REFERENCE TO RELATED APPLICATIONS

The present Application claims priority to U.S. Provisional Application Ser. No. 61/531,471 filed Sep. 6, 2011, the entirety of which is incorporated by reference herein.

STATEMENT REGARDING FEDERALLY SPONSORED RESEARCH OR DEVELOPMENT

This invention was made with government support under 1R43AI077156-01 awarded by the National Institutes of Health. The government has certain rights in the invention.

FIELD OF THE INVENTION

The present invention provides whole blood nucleic acid extraction methods, compositions, and kits, as well as nested isothermal amplification methods, compositions, and kits. In certain embodiments, these methods are applied to detecting Lyme disease, including in patients without classic erythema migrans skin lesions.

BACKGROUND

The diagnosis of acute infectious diseases is problematic when the pathogens are not in abundance, not easily cultured or the antibody response to them is delayed. Lyme disease is such an example. Infection by the causative agent, Borrelia burgdorferi ^(1,2), is often difficult to diagnose because of clinical variability, including variations of the erythema migrans (EM) skin lesion and the lack of high performing diagnostic tests. A strategy that results in early unambiguous diagnosis of the infection will favorably impact management of the patient.

There are currently clinical limitations to early diagnosis. The best clinical marker of acute infection, the skin lesion erythema migrans (EM), is absent in at least 30% of the cases.³ Even when present, the EM is often not the classic bull's-eye lesion but rather an uncharacteristic variant as reported in 25-30% of cases.^(4,5) This may require referral to a specialist or prompt further diagnostic testing, thereby delaying the start of antibiotic therapy at the time for the best chance of cure without sequelae.

These clinical hurdles to diagnosis are compounded by the limitations of current laboratory tests. The most commonly used assays are serologic. However, these assays have been hampered by the biologically delayed antibody response (often 3 weeks or more to reach detectable levels). They are further limited because a single positive test is an indirect measure of exposure and cannot distinguish active from past infection. A direct Borrelia molecular test such as PCR can have high specificity but typically the tests have lacked sensitivity when applied to blood. In the past, PCR assays for Lyme disease did not have the benefit of current advances in sample preparation.⁶ and enhancement methods.^(7,8) such as Borrelia-targeted DNA enrichment (akin to a “molecular culture”) that may allow detection of a low number of nucleic acid copies in the blood. In addition, the optimal blood volume and component of the sample, such as whole blood versus serum, may have contributed to prior limitations of PCR based diagnostics.

SUMMARY OF THE INVENTION

The present invention provides whole blood nucleic acid extraction methods, compositions, and kits, as well as nested isothermal amplification methods, compositions, and kits. In certain embodiments, these methods are applied to detecting Lyme disease, including in patients without classic erythema migrans skin lesions.

In some embodiments, the present description provides methods of nucleic acid extraction comprising: a) contacting a sample of whole blood (e.g., EDTA treated whole blood) with beads, a proteinase, and an anionic surfactant (e.g., SDS) to generate a treated sample; b) homogenizing the treated sample to generate a cell lysate; c) centrifuging the cell lysate comprising a supernatant; d) separating the supernatant from the cell lysate; e) adding magnetic particles and lysis buffer to the supernatant to generate a magnetic-particle sample, wherein the magnetic particles are configured to bind nucleic acid molecules; f) washing the magnetic-particle sample with a wash buffer; g) treating the magnetic-particle sample in order to generate a dried magnetic bead sample; and h) treating the dried magnetic bead sample with an elution buffer such that a purified nucleic acid sample is generated that comprises purified nucleic acid.

In certain embodiments, the methods further comprise subjecting the purified nucleic acid to PCR and/or isothermal nested PCR to generate amplified nucleic acid. In some embodiments, the methods further comprise subjecting the amplified nucleic acid to mass spectrometry bioagent analysis in order to identify the source of the purified nucleic acid. In other embodiments, the mass spectrometry bioagent analysis comprises electrospray ionization mass spectrometry and base composition analysis.

In some embodiments, the present disclosure provides methods comprising: a) contacting a sample comprising isolated nucleic acid with a buffer, dNTPs, and a plurality of nested PCR primer pairs configured to amplify at least part of at least one bioagent target sequence; b) incubating the sample with a DNA polymerase under isothermal conditions such that amplified nucleic acid is generated; c) inactivating the DNA polymerase; and d) subjecting the amplified nucleic acid to mass spectrometry bioagent analysis in order to identify the source of the isolated nucleic acid.

In other embodiments, the mass spectrometry bioagent analysis comprises electrospray ionization mass spectrometry and base composition analysis. In certain embodiments, the DNA polymerase comprises BstE DNA polymerase. In additional embodiments, the incubating is conducted at about 56 degrees Celsius. In further embodiments, inactivating the DNA polymerase comprises heating the sample to at least about 80 degrees Celsius. In other embodiments, the plurality of nested PCR primer pairs comprises at least 10 primer pairs (e.g., 10 . . . 15 . . . 19, etc). In particular embodiments, the plurality of nested PCR primer pairs comprises at least 20 primer pairs (e.g., 20 . . . 25 . . . 35 . . . 45 . . . etc.). In further embodiments, the at least one bioagent target sequence comprises at least five bioagent target sequences. In certain embodiments, the methods further comprise a step after c) but before d) of further amplifying the amplified nucleic acid without any purification of the amplified nucleic acid.

DESCRIPTION OF THE FIGURES

FIG. 1 shows an atypical EM lesion from a patient who was PCR positive and seronegative with a negative ELISA after eight days of illness. Repeat serology at the end of therapy 3 weeks later showed a positive ELISA, positive IgM western blot and negative IgG western blot.

DETAILED DESCRIPTION

The present invention provides whole blood nucleic acid extraction methods, compositions, and kits, as well as nested isothermal amplification methods, compositions, and kits. In certain embodiments, these methods are applied to detecting Lyme disease, including in patients without classic erythema migrans skin lesions.

The methods, kits, and compositions are useful with any target nucleic acid sequence and are not limited to any particular target sequence (e.g., not limited to nucleic acid sequences from B. burgdorferi). The discussion below is focused on detecting sequence from B. burgdorferi. Such target sequences are exemplary and are not intended to limit the scope of the present description. Other target sequences (e.g., from infections disease) are well known in the art. Also well know in the art are primers, including nested prior sets, that are useful in the present description.

Lyme disease is representative of an infectious disease where early diagnosis is imperative to avoid sequelae. However diagnosis is often difficult because the clinical manifestations, including the rash, are variable and the pathogens are often not in abundance, not easily cultured, and the antibody response to them is delayed. In the past PCR for B. burgdorferi in blood had low sensitivity. This may be related to low copy number, insufficient volume of blood or targeting the wrong component of blood

The present description overcomes some of these obstacles by combining a pre-PCR nucleic acid enrichment with sensitive PCR detection from nucleic acid extraction from 1.25 ml of whole blood from patients with skin lesions and early Lyme disease. With this strategy, PCR positivity was found in 14 of 29 (p=0·0001) endemic area subjects with typical erythema migrans (EM) or a variant, often before seroconversion was positive. The enrichment technique increased the yield from 2 to 14. None of 44 control subjects were positive. A serendipitous and unexpected finding of clinical importance was the observation that 8 of 14 (57%) of PCR positive subjects had an atypical EM.

The description provides improved early diagnosis of Lyme disease by combination of a pre-PCR Borrelia DNA enhancement, sensitive PCR, and targeting sufficient volumes of whole blood. The surprise finding of non-classic EM lesions in the majority of microbiologically proven Lyme disease cases serves as alert to clinicians evaluating patients with endemic area exposure.

In certain embodiments, the PCR generated amplicons are detected by mass spectrometetry methods using bioagent identifying amplicons. In some embodiments, primers are selected to hybridize to conserved sequence regions of nucleic acids derived from a bioagent and which flank variable sequence regions to yield a bioagent identifying amplicon which can be amplified and which is amenable to base composition analysis. In some embodiments, the corresponding base composition of one or more different amplicons is queried against a database of base compositions indexed to bioagents and to the primer pair used to generate the amplicon. A match of the measured base composition to a database entry base composition associates the sample bioagent to an indexed bioagent in the database. Thus, the identity of the unknown bioagent is determined. No prior knowledge of the unknown bioagent is necessary to make an identification. In some instances, the measured base composition associates with more than one database entry base composition. Thus, a second/subsequent primer pair is generally used to generate an amplicon, and its measured base composition is similarly compared to the database to determine its identity in triangulation identification. Furthermore, the methods and other aspects of the invention can be applied to rapid parallel multiplex analyses, the results of which can be employed in a triangulation identification strategy. Thus, in some embodiments, the present invention provides rapid throughput and does not require nucleic acid sequencing or knowledge of the linear sequences of nucleobases of the amplified target sequence for bioagent detection and identification.

Methods of employing base compositions, databases containing base composition entries, and triangulation using primers, are described in the following patents, patent applications and scientific publications, all of which are herein incorporated by reference as if fully set forth herein: U.S. Pat. Nos. 7,108,974; 7,217,510; 7,226,739; 7,255,992; 7,312,036; 7,339,051; US patent publication numbers 2003/0027135; 2003/0167133; 2003/0167134; 2003/0175695; 2003/0175696; 2003/0175697; 2003/0187588; 2003/0187593; 2003/0190605; 2003/0225529; 2003/0228571; 2004/0110169; 2004/0117129; 2004/0121309; 2004/0121310; 2004/0121311; 2004/0121312; 2004/0121313; 2004/0121314; 2004/0121315; 2004/0121329; 2004/0121335; 2004/0121340; 2004/0122598; 2004/0122857; 2004/0161770; 2004/0185438; 2004/0202997; 2004/0209260; 2004/0219517; 2004/0253583; 2004/0253619; 2005/0027459; 2005/0123952; 2005/0130196 2005/0142581; 2005/0164215; 2005/0266397; 2005/0270191; 2006/0014154; 2006/0121520; 2006/0205040; 2006/0240412; 2006/0259249; 2006/0275749; 2006/0275788; 2007/0087336; 2007/0087337; 2007/0087338 2007/0087339; 2007/0087340; 2007/0087341; 2007/0184434; 2007/0218467; 2007/0218467; 2007/0218489; 2007/0224614; 2007/0238116; 2007/0243544; 2007/0248969; WO2002/070664; WO2003/001976; WO2003/100035; WO2004/009849; WO2004/052175; WO2004/053076; WO2004/053141; WO2004/053164; WO2004/060278; WO2004/093644; WO 2004/101809; WO2004/111187; WO2005/023083; WO2005/023986; WO2005/024046; WO2005/033271; WO2005/036369; WO2005/086634; WO2005/089128; WO2005/091971; WO2005/092059; WO2005/094421; WO2005/098047; WO2005/116263; WO2005/117270; WO2006/019784; WO2006/034294; WO2006/071241; WO2006/094238; WO2006/116127; WO2006/135400; WO2007/014045; WO2007/047778; WO2007/086904; WO2007/100397; and WO2007/118222, all of which are herein incorporated by reference.

Exemplary base-count related methods and other aspects of use in the methods, systems, and other aspects of the invention are also described in, for example, Ecker et al., Ibis T5000: a universal biosensor approach for microbiology. Nat Rev Microbiol. 2008 Jun. 3.; Ecker et al., The Microbial Rosetta Stone Database: A compilation of global and emerging infectious microorganisms and bioterrorist threat agents.; Ecker et al., The Ibis T5000 Universal Biosensor: An Automated Platform for Pathogen Identification and Strain Typing.; Ecker et al., The Microbial Rosetta Stone Database: A common structure for microbial biosecurity threat agents.; Ecker et al., Identification of Acinetobacter species and genotyping of Acinetobacter baumannii by multilocus PCR and mass spectrometry. J Clin Microbiol. 2006 August; 44(8):2921-32.; Ecker et al., Rapid identification and strain-typing of respiratory pathogens for epidemic surveillance. Proc Natl Acad Sci USA. 2005 May 31; 102(22):8012-7. Epub 2005 May 23.; Wortmann et al., Genotypic evolution of Acinetobacter baumannii Strains in an outbreak associated with war trauma, Infect Control Hosp Epidemiol. 2008 June; 29(6):553-555.; Hannis et al., High-resolution genotyping of Campylobacter species by use of PCR and high-throughput mass spectrometry. J Clin Microbiol. 2008 April; 46(4): 1220-5.; Blyn et al., Rapid detection and molecular serotyping of adenovirus by use of PCR followed by electrospray ionization mass spectrometry. J Clin Microbiol. 2008 February; 46(2):644-51.; Eshoo et al., Direct broad-range detection of alphaviruses in mosquito extracts, Virology. 2007 Nov. 25; 368(2):286-95.; Sampath et al., Global surveillance of emerging Influenza virus genotypes by mass spectrometry. PLoS ONE. 2007 May 30; 2(5):e489.; Sampath et al., Rapid identification of emerging infectious agents using PCR and electrospray ionization mass spectrometry. Ann N Y Acad Sci. 2007 April; 1102: 109-20.; Hujer et al., Analysis of antibiotic resistance genes in multidrug-resistant Acinetobacter sp. isolates from military and civilian patients treated at the Walter Reed Army Medical Center. Antimicrob Agents Chemother. 2006 December; 50(12):4114-23.; Hall et al., Base composition analysis of human mitochondrial DNA using electrospray ionization mass spectrometry: a novel tool for the identification and differentiation of humans. Anal Biochem. 2005 Sep. 1; 344(1):53-69.; Sampath et al., Rapid identification of emerging pathogens: coronavirus. Emerg Infect Dis. 2005 March; 11(3):373-9.; Jiang Y, Hofstadler S A. A highly efficient and automated method of purifying and desalting PCR products for analysis by electrospray ionization mass spectrometry; Jiang et al., Mitochondrial DNA mutation detection by electrospray mass spectrometry; Russell et al., Transmission dynamics and prospective environmental sampling of adenovirus in a military recruit setting; Hofstadler et al., Detection of microbial agents using broad-range PCR with detection by mass spectrometry: The TIGER concept. Chapter in; Hofstadler et al., Selective ion filtering by digital thresholding: A method to unwind complex ESI-mass spectra and eliminate signals from low molecular weight chemical noise.; Hofstadler et al., TIGER: The Universal Biosensor.; Van Ert et al., Mass spectrometry provides accurate characterization of two genetic marker types in Bacillus anthracis.; Sampath et al., Forum on Microbial Threats: Learning from SARS: Preparing for the Next Disease Outbreak—Workshop Summary (ed. Knobler S E, Mahmoud A, Lemon S.) The National Academies Press, Washington, D.C. 2004. 181-185.

EXAMPLES Examples 1 Early Lyme Patient Specimens.

The current Example is part of a larger, ongoing longitudinal cohort study of early Lyme disease being conducted in a suburban community of a medium-sized, Northeast city since the summer of 2008. Adult patients with early, untreated Lyme disease are referred to a primary care physician with infectious disease training (JA) and provide written consent to participate.

Eligible patients are required to be treatment naïve, to have a documented rash diagnosed as EM at time of enrollment, and to have evidence of systemic infection; typically manifest as dissemination of the primary EM lesion or concurrent onset of new flu-like or other symptoms. Patients with a prior history of Lyme disease or symptom duration of their current illness of longer than 3 months are excluded.²⁰. Forty four negative control specimens were obtained from Biomed Supply Inc. (Carlsbad, Calif.). Specimens were collected at a donation site in Pennsylvania from healthy donors screened by Biomed Supply Inc. A paired 7 mL tube of EDTA treated whole blood and 5-12 mL of serum was provided for each control patient.

Serological and Other Analyses.

At the initial, pre-treatment study visit, self-report demographics, medical history information, complete blood counts (CBC), complete metabolic panels (CMP) and 2-tier antibody testing for B. burgdorferi were performed as part of the patient clinical evaluation. All serologic testing for both the patient specimens and the negative controls was performed through the same commercial laboratory, and results were interpreted according to CDC criteria¹¹. Based on these criteria, approximate illness duration was documented and included in determining serostatus; patients with less than 4 weeks illness duration were positive based on either IgM or IgG positivity on western blot analysis, whereas patients with greater than 4 weeks illness duration were required to be IgG positive. Photos of EM rashes were reviewed by a panel of experienced clinicians without knowledge of serologic or PCR status. Skin lesions with classic bull's eye appearance with central clearing and peripheral erythema were classified as classic EM lesions. EM with uniform red or red-blue appearance which lacked central clearing were classified as non-classic EM lesions.

DNA Extraction from Blood Specimens:

A combination of bead-beating and magnetic bead isolation was used to extract nucleic acids from 1.25 mL of whole EDTA blood. The blood was mixed in 2.0 mL screw-cap tubes (Sarstedt, Newton N.C.) filled with 1.35 g of 0.1-mm yttria-stabilized zirconium oxide beads (Glen Mills, Clifton, N.J.), 25 μL proteinase K solution (Qiagen, Valencia, Calif.), 142 μL of 20% SDS solution (Ambion, Austin, Tex.) and 1 uL of DNA extraction control (Abbott Molecular, Des Plains, Ill.). The mixture was then homogenized in a Precellys 24 tissue homogenizer (Bioamerica Inc., Miami, Fla.) at 6,200 rpm for 3 sets of 90 sec with 5 sec between sets. The homogenized lysates were then incubated at 56° C. for 15 min and then centrifuged for 3 min at 16,000 g in a bench top microcentrifuge. To isolate nucleic acids 1 mL of the supernatant was transferred to a 24-well deep-well Kingfisher plate (Thermo Scientific, Waltham, Mass.) along with 1.1 mL of Abbott lysis buffer (Abbott Molecular), and 160 μL of magnetic particles (Abbott Molecular). The specimens were incubated for 16.5 minutes in the lysis buffer at 56° C. Specimens were then washed once in Wash buffer I (Abbott Molecular), and three times in Wash buffer II (Abbott Molecular), with 1 min incubation for each wash step. The magnetic beads were then dried for 3 min at 65° C., and nucleic acids were eluted into 250 μL of elution buffer (Abbott Molecular), by incubating the magnetic particles at 65° C. for 3 min.

Nested Isothermal Amplification of B. burgdorferi Target DNA.

To increase sensitivity of B. burgdorferi detection by PCR/ESI-MS the seven target regions (eight primer pairs) of the previously described Borrelia genotyping assay²¹ were enriched by a nested isothermal amplification. For each of the seven target regions were amplified using 50 oligonucleotide primers: 25 upstream and 25 downstream to the DNA region of interest (Table 1).

TABLE 1 Primer Pair Gene  Target Target Primer Sequence 3′-5′ BCT3514 rpoC 3514E3-F1 CCGAAAAAGATGGGCTTTT 3514E3-F2 AGGTTAAAAAGTCCGAAACTATT 3514E3-F3 TCTCCCGATCAAATTAGAAATTG 3514E3-F4 AAAGAGATAAAAGATTTTGAAAGAATAAA 3514E3-F5 AAAGCTAGGTTTTTGGAGTTTT 3514E3-F6 ACAGAAAAAGAAGAAGAATTGATTAA 3514E3-F7 ATGATGCTGGGAATCAGGTTC 3514E3-F8 GGGCTTGGACTTGATTTG 3514E3-F9 GTCTTTTAATGTGCTAATGCAAGA 3514E3-F10 GGTTCCTACTAATGTATCAGGG 3514E3-F11 GGCAGAGTTAAAATATATGAAAATATAG 3514E3-F12 CACCCTTCAAGAACTTTTAACAG 3514E3-F13 GGCTCTTGAAGCTTATGG 3514E3-F14 AGACTTGGAGAAATGGAGG 3514E3-F15 GAGGAAAGGCTCAATTTGG 3514E3-F16 TCTTGTTTCTCAGCAACCT 3514E3-F17 CGCAAGATCAACAGGC 3514E3-P18 ACTACACCATCTTGTTGATGATA 3514E3-F19 GTAATGGTTGGGGTGATTTAC 3514E3-F20 GGAGAGCCGTTCGAAA 3514E3-F21 CCAACTTCTAAAGAAATTTTATATGATGG 3514E3-F22 AGGAAAAATTAAAAACTGCTGGA 3514E3-F23 TGTTTTTGAATCTGCTACAAATGA 3514E3-F24 CTGGTAAATATCTTGGTGAATCTTATAA 3514E3-F25 GGACAGTTAATGGAATCTCAAT 3514E3-R1 ATACCAAATATGAGCAACTGGGGC 3514E3-R2 AAGCCCAATCCTAGAGGGTA 3514E3-R3 TAGAATTCAAACTAGATGCTGTAAT 3514E3-R4 GCCTTCAATTACTACATATTTTTCATA 3514E3-R5 GGCCGGTTCAATTACTACA 3514E3-R6 TCTTCATTTAAAAGCTGCATTTTT 3514E3-R7 GCTCTCTAGCTTCTATGTACTCA 3514E3-R8 AAGCATTAAAAGACATACCATATCGC 3514E3-R9 GAAGAGTTTTAATAGCCTCAGCCC 3514E3-R10 GACGAAAGCTCATCAAGATCA 3514E3-R11 CAGTTTTATCATCTTTATCTATCATTTGAA 3514E3-R12 AAATTCTCAATAATTTCAAGACGTCTT 3514E3-R13 ATCCACTCTGGCTTATTGCCA 3514E3-R14 GGGGAATAACAGGAAGAAC 3514E3-R15 GCTGAACCATTGGCC 3514E3-R16 ATGTTGCAAAGCGCC 3514E3-R17 CGATTATTTCTATTTATGACTCTTCTATAAAGATC 3514E3-R18 GCATTAAGAAGAAGCAACTTTCT 3514E3-R19 ATTCTTTTTTCGTTTCTCACAATAATC 3514E3-R20 GTCAAAAAGAGAGTCTACTGATTC 3514E3-R21 GAACCTTTGACAACCTTTCTTTTA 3514E3-R22 CGACTTGAGAGGCCT 3514E3-R23 CCTGCTTACCTTTTAATGCAT 3514E3-R24 TTTTACCAAGAAGATTTTGCCTAA 3514E3-R25 CAATAACAGAACGACCAGAATAA BCT3515 rplB 3515E3-F1 GTGTTGCTATGAATCCTGTTG 3515E3-F2 GGTAGAAGACCCAAGGT 3515E3-F3 GGAAAGCTGGTAAAAGTAGG  3515E3-F4 TGGAAATGAAGATTATGCCAATATTT 3515E3-F5 TTTTAAAAAATGTATTGCAACAATTGG 3515E3-F6 TTATCATCTGGCGAGATGAG 3515E3-F7 GACGGGAATTATGTCACTG 3515E3-F8 GGTGGATATGCTATGATACTTG 3515E3-F9 GGGTGGACAGCTTATAAGA 3515E3-F10 CGTTCACAATATTGAGCTTAATGT 3515E3-F11 CTTACCTCTTGAAAATATTCCTATTGG 3515E3-F12 CTAATGCTCCAATTAAAATTGGC 3515E3-F13 GGTTGGAGATGTTTTGGAAAG 3515E3-F14 AAAGGTATATTATTTCTCCTAAAGGC 3515E3-F15 GCTAATATAGCTTTGCTTGTTTATAAAG 3515E3-F16 GTTGCTTCTATTGAATATGATCCTAA 3515E3-F17 CGAAGAGATAAATTTAGCATTCCTG 3515E3-F18 GCATAAGAGAAAGTATAGGTTGATTG 3515E3-F19 CTGGTAGGATTAGTATTAGAAGAAGAG 3515E3-F20 AAAAGGTAAAAAATTTAAATCGGGC 3515E3-F21 CAAAGGTAATGATCCTTTGAAATC 3515E3-F22 GCTATAAGACGACTTTATCTTTTGAT 3515E3-F23 AGACTTATAAGCCAAAAACTTCTTC 3515E3-F24 GGTTTTGGAGAAAAATAAATATGGG 3515E3-F25 CAAAAAGGAAGATAAAATAGATATTTTTTAGTC 3515E3-R1 TTTCTTGCGAGTCTTATAACCT 3515E3-R2 TTTATTTCTTCTTTTAATAATAAATTTATCTGAATATC 3515E3-R3 TTTTTTAATAGATCTTGCCACTATACTC 3515E3-R4 ACTTTTTGATAAAGACTCTTTTCTATAAAAG 3515E3-R5 CTTCTCACTTCCAAAAGACG 3515E3-R6 AAGATCTGGAGTAGGTTTTAATAAC  3515E3-R7 GGCTTACCATTTCAGGAATTAT 3515E3-R8 AAGTTTTGCCATTGTAAACAGATAT 3515E3-R9 CAAGATCCTCGGTAATATAAATAGGT 3515E3-R10 CTCGCCAAGCTTATGTC 3515E3-R11 CCTCTAAAAATCCTTGTAGGTG 3515E3-R12 CCTCTAAAAATCCTTGTAGGTG 3515E3-R13 CTTCCCTTTTTATCTGACTTAGC 3515E3-R14 ATCTTCTATTTACCAACATAACTACTTAC 3515E3-R15 AGGGTAAATTTTTGCCCTTTG 3515E3-R16 CTATTGGCCTAACTTTTTTTGG 3515E3-R17 AGACTCTCCCCGGATATT 3515E3-R18 AAAGCACTGCAATAGCC 3515E3-R19 TAAAAGCTTAGCTCCTTTATTAGG 3515E3-R20 TGATGCTGCTGACTTAACAA 3515E3-R21 CTCGGAAAGATTTTTATTGTGATACA  3515E3-R22 CATCAACCATAACTGTTTTAACAAATATC 3515E3-R23 GCCAAATCTTTTTACGACGAC 3515E3-R24 TATCAGCTCTACCCCTAGC 3515E3-R25 CTTCAACAAAAATATGACAATTTCTATTAAC BCT3516 leuS 3516E3-F1 CCTATCCTTCTGCCAACG 3516E3-F2 GGAAAAAAGATTGTATATACTTGACATG 3516E3-F3 CAAAGTAGAAGAAGATCCAAGTATTC 3516E3-F4 GGCAAGAATTTTGGGATAATAACA 3516E3-F5 TGTCTAAATACGAATTCATAAAAATTGAAA 3516E3-F6 GAATAAGTTGTTATGAGTTAATTTTCAAGA 3516E3-F7 TAAATAAAATTAACAAAAATGCAATCTAAAAGAA 3516E3-F8 CACAGCATCAAAATTGTTAGC 3516E3-F9 CCGTGCTGGTTCAAG 3516E3-F10 GAGGGGCTAGTGGG 3516E3-F11 GGAAGTGGTAGACACGC 3516E3-F12 AAAAAATATAATGGTTAATAGTGCTGTG 3516E3-F13 GTAATTAAAAAAAATAAAAAAGTTGACAAAAATT 3516E3-F14 CGCTGTAATAGCAACAACAATAATA 3516E3-F15 AATAATATTTTCAAAAATAAAAATAATTATATTTGCAA 3516E3-F16 CTCTAAGCTTCAAACTAGGTCA 3516E3-F17 AACTTTGCTCTCAATAGTTGTTT 3516E3-F18 TATGAAATCTAATCTATTTATTGTTTCTGACT 3516E3-F19 GCAATATTTATGTCAGCAGGAA 3516E3-F20 GAAGGTTTATACCCTTTGGAG 3516E3-F21 TGGTCAATATGGGGTATTAACTTTAT 3516E3-F22 CAATAACCTGCTTGACAAAATAAATTA 3516E3-F23 GGAAATTAATGGGAAATAAATTATTTAAAAACA 3516E3-F24 AGACATAATATCTTTTTACATTGGGAAA 3516E3-F25 TTTAGGAATTTTTTGGGGAGC 3516E3-R1 TGAGGGTGAGTTCCTGT 3516E3-R2 TTGTTTTTTAAACTTATTAATATTTTCTTCTGTAC 3516E3-R3 GGCAAACCCCAAAGC 3516E3-R4 GTGTTCTAATTTCTCGATCCC 3516E3-R5 ACTGTGTCCATTTATAGTAATTCTC 3516E3-R6 CTAGCCCTTTTTTATATAATTGCAGG 3516E3-R7 GTACCATACAGGCATTTCTTTTA 3516E3-R8 CTAGTACCGTTCCAAGCT 3516E3-R9 GTCCATCTGAAGTTTGAATAATCTC 3516E3-R10 ACGCTGTAAGATCCTCTC 3516E3-R11 GTAATTTTTAAAACCCACTGTCTTAAATA 3516E3-R12 CGTCTAGCAATCTTTCAGC 3516E3-R13 AGATTCAGGCCATTCTAATTCT 3516E3-R14 TCCAATTTCGCTGCATTTC 3516E3-R15 AATTCAATTTCAACTCCTGTTGAT 3516E3-R16 TTTTATCGCTGTGGCCTT 3516E3-R17 CTTTACAACAAGGCCAGAC 3516E3-R18 CGATCACTAAATATGTGATGCC 3516E3-R19 GTTGTTCTTTGTTATTTTTTCTATTAGTTTATT 3516E3-R20 CTTCGTGCTTTACATATTTTAAAACATT 3516E3-R21 GAGAAGTCCTATTAAGATCGCT 3516E3-R22 CTGTGAAAACTCCCGATTTATC 3516E3-R23 CATTTGTTATTGGATGAAATGCG 3516E3-R24 GCTTCCAACCCAAATTG 3516E3-R25 CGGTTCCGTAAGTTCCT BCT3517 flaB 3517E3-F1 TCTGCTTCTCAAAATGTAAGAACA 3517E3-F2 TAACCAAATGCACATGTTATCAAA 3517E3-F3 TTGCTGATCAAGCTCAATAT 3517E3-F4 GCAACTTACAGACGAAATTAAT 3517E3-F5 AGACAGAGGTTCTATACAAATTGA 3517E3-F6 AGGTAACGGCACATATTCAGA 3517E3-F7 TAAGAATGAAGGAATTGGCAGTT 3517E3-F8 AATTTAAATGAAGTAGAAAAAGTCTTAGT 3517E3-F9 GGCTATTAATTTTATTCAGACAACAGA 3517E3-F10 TTGTCACAAGCTTCTAGAAATA 3517E3-F11 TTTCTGGTAAGATTAATGCTCAAAT 3517E3-F12 GAGCTTCTGATGATGCTGCT 3517E3-F13 GAAAAGCTTTCTAGTGGGTAC 3517E3-F14 CATTAACGCTGCTAATCTTAGTAA 3517E3-F15 CATCAGCTATTAATGCTTCAAGA 3517E3-F16 CATGGAGGAATGATATATGATTATCATG 3517E3-F17 TTTTTTTTTAATTTTTGTGCTATTCTTTTTAAC 3517E3-F18 TAATAATAATTATTTTTAATGCTATTGCTATTTGC 3517E3-F19 ATTAAAGGCTTTTGATTTTAATCAAAGA 3517E3-F20 TTAAGCGCATGAAAGATCAAG 3517E3-F21 GTGGAAGGTGAACTTAATACC 3517E3-F22 GATTATAAAAAGAAGTACGAAGATAGAGAG 3517E3-F23 TTATTTTTTTGATTAAAAATTTTCAAGTCGTAA 3517E3-F24 GCTTCCGGAGGAGTTATTTAT 3517E3-F25 TAGGAGATTGTCTGTCGC 3517E3-R1 GCAACATTAGCTGCATAAATAT 3517E3-R2 TCCCTCACCAGAGAAAG 3517E3-R3 ACACCCTCTTGAACCGGTG 3517E3-R4 TGAGAAGGTGCTGTAGCAGG 3517E3-R5 TTGTAACATTAACAGGAGAATTAACTC 3517E3-R6 TTAGCAAGTGATGTATTAGCATCA 3517E3-R7 TGATCACTTATCATTCTAATAGCATTT 3517E3-R8 CTATTTTGGAAAGCACCTAAAT 3517E3-R9 GCATACTCAGTACTATTCTTTATAGAT 3517E3-R10 TGAGCATAAGATGCTTTTAGATTT 3517E3-R11 TCTGTCATTGTAGCATCTTTTA 3517E3-R12 TTAAAATACTATTAGTTGTTGCTGCTAC 3517E3-R13 ATTAGCCTGCGCAATCAT 3517E3-R14 GCAATGACAAAACATATTGGG 3517E3-R15 TTAATACAATTTATACCAATTAAACTAGAATTTT 3517E3-R16 ATAAAAAAACAAAAGATCCTTTAAAGGATC 3517E3-R17 ATAAATTATACTAAAATTATTAAATTTTTGCCGAT 3517E3-R18 GCCTGCATTATGCTTTATAACA 3517E3-R19 CCTACTCAAAGCAAACTCC 3517E3-R20 CGAAAATACTTTATAACAATCTTTAATTTTAACA 3517E3-R21 TCGACTTATCTGCTTTTTGTTAAC 3517E3-R22 CTATCTTTGCCATCTTCATAGTC 3517E3-R23 GCAATAAAAATAGAAGATTCTTTGTAGAT 3517E3-R24 TAAAATTTCATTTTCATAAACATCAAGATTAATA 3517E3-R25 GCCCGACATACCCA BCT3518 ospC 3518E3-F1 TTAATGAAAAAGAATACATTAAGTGCAATAT 3518E3-F2 CTAATAATTCATAAATAAAAAGGAGGCAC 3518E3-F3 TTTTCAAATAAAAAATTGAAAAACAAAATTGT 3518E3-F4 AATATTTATTCAAGATATTGAAGAATTTGAAAAA 3518E3-F5 TTTAAAATCAAATTAAGACAATATTTTTCAAATTC 3518E3-F6 AGCATATTTGGCTTTGCTTATG 3518E3-F7 AAATTAAAACTTTTTTTATTAAAGTATACTTCATTTAA  3518E3-F8 GCCTGAGTATTCATTATATAAGTCC 3518E3-F9 TATATTGGGATCCAAAATCTAATACAAG 3518E3-F10 CAATTTCTCTAATTCTTCTTGCAATTAG 3518E3-F11 GGAGTATAGTAAGGTATTACTTTTGTATAAA 3518E3-F12 TTCCTGAGATATTCATATTTTTAATTTCTTTT 3518E3-F13 GCAGGACTTCCACTTAGTA 3518E3-F14 GGTAGGAGCTTCTTTTGAATAAAC 3518E3-F15 CAAAATAGGTATTTTCAAATTAAAAATTTCCATA 3518E3-F16 AATTTAACAATTATTTGCATTCCATAACATA 3518E3-F17 GCTTAGAGTCTTTAGATACTAGGC 3518E3-F18 AAAGATTTCAGAGCTCCCATAT 3518E3-F19 TTCTGAAAATAAAAGAGATTTTTCATCTC 3518E3-F20 TGACTCATGATAATTTGAAATTTGTTTG 3518E3-F21 AAATTATCAGGCCTTTTTTCAATACTGTC 3518E3-F22 GCAATACAATTTTTTGTAAAAGCTAATTG 3518E3-F23 CCGTAAATTTTTTGAGTTTCATTTGAT 3518E3-F24 AGTTACTTCTGGATGGAATTGT 3518E3-F25 AATTTTTAATTATTTGATCACCAAATTCAG 3518E3-R1 ACCGCATTAGAATCCGTAAT 3518E3-R2 ACCTCTTTCACAGCAAGTT 3518E3-R3 CATCTATAGATGACAGCAACG 3518E3-R4 TTACCAATAGCTTTAGCAGCA 3518E3-R5 GTATCCAAACCATTATTTTGGTGTA 3518E3-R6 GCTAACAATGATCCATTGTGATTAT 3518E3-R7 TATTAGGGTTGATATTGCATAAGC 3518E3-R8 CTTCATTTTTCAATCCATCTAATTTTTG 3518E3-R9 TTAGCCGCATCAATTTTTTCC 3518E3-R10 TCTTTTAATTTATTAGTAAATGTTTCAGAACA 3518E3-R11 CTTCTTTACCAAGATCTGTGTG 3518E3-R12 CTTTTGCATCAGCATCAGT 3518E3-R13 TTTAGTTTTAGTACCATTTGTTTTTAAAATG 3518E3-R14 GATTCAAATAATTTTCCAAGTTCTTCAG 3518E3-R15 CTGCTTTTGACAAGACCTC 3518E3-R16 TTTAACTGAATTAGCAAGCATCTC 3518E3-R17 CCACAACAGGGCTTG 3518E3-R18 GATCTTAATTAAGGTTTTTTTGGACTT 3518E3-R19 CCAGTTACTTTTTTAAAACAAATTAATCTTATA 3518E3-R20 AGAAATCTTTCTTGACTTATATTGACTTT 3518E3-R21 GAATTTTAAGAAATTTTTTGAGAAAATAAAAAAATAAAA 3518E3-R22 TATTCTTTAAGAGAAGAGCTTAAAGTT 3518E3-R23 AAATTCAATTTATTAACGGCTTTTGTAATA 3518E3-R24 TCTAGCACCCAATTTTGTTTATATTTA 3518E3-R25 GTTTAAGCCTACTTAAAGTCTTTAAAATC BCT3519 hbb 3519-20E3-F1 CCCACACTCTCTCTTTCAAA and 3519-20E3-F2 GATATTAACCGGCATTTAACCTT BCT3520 3519-20E3-F3 TCTAGCTTACAATCCCATTTATAAGA 3519-20E3-F4 CCTTCAAATTTTAATTTTCCTCTAAAAGTTA 3519-20E3-F5 CCTTCAAAAGAAGAATCAAGATACAA 3519-20E3-F6 CACACCCCCTTTTGAAGATA 3519-20E3-F7 GTAATAACCTTACTATTCTTGCCAATA 3519-20E3-F8 TTCTACTATTAATGTATCACAAATTACCAC 3519-20E3-F9 GCATTTACATTGCCCTTCAA 3519-20E3-F10 CAACCGCTGTTTAAATAAACCTT 3519-20E3-F11 AATATTTTTTTTGTTTTTACATCCCCATAT 3519-20E3-F12 CACACTTACCATCAAAAATTATATTATCAT 3519-20E3-F13 AAGAAAATAAATCTACAATTTCATTAGACTTTA  3519-20E3-F14 CAAAGTATCTTTTATTTGTGAAACGG 3519-20E3-F15 TCTACTTATTATTAATTAATAAAAAACACTGACC 3519-20E3-F16 CTCTACGAATTAAATTTTTAAGAAAGGATTTTA 3519-20E3-F17 ATCAAATCCACCATTTTTTTTATCCA 3519-20E3-F18 CCAACCGCCTTATTTCAC 3519-20E3-F19 TTTTCAAATTATCTTCAATCTTAAACTCTTTAG 3519-20E3-F20 TTTTAGCAACAACTTTAACCACTTT 3519-20E3-F21 TGTCACGCTAGATGCAG 3519-20E3-F22 CTTTACGCCACTTAAATCTGC 3519-20E3-F23 AATCAGAAAATATTACCCCGTTTG 3519-20E3-F24 ATATTATTTTCTAAACCTGAAGAAGGAATAT 3519-20E3-F25 CATTAAAAAATTTGATGATATTACTTTGCTC 3519-20E3-R1 GTTTTGCTGTTAAAGTAAGGAAATTAG 3519-20E3-R2 GCTGCTAGAAAAAAATCTCGTT 3519-20E3-R3 CTGCTAGAAAGCGAATAATTCATAA 3519-20E3-R4 GAATTTTTTAAATTTGTTGCAAAAAAACTAG 3519-20E3-R5 GCGGGTAAGAAAGACGAA 3519-20E3-R6 GAAAAACGCTGTATCAACATGA 3519-20E3-R7 ATTAGAAATGTAAGTGTAAAAAGTGAATTAAAA 3519-20E3-R8 CGCTCTCGTCAAAATTTAAAAAG 3519-20E3-R9 CTTGAGAAAAAATGCATCTGC 3519-20E3-R10 GATATATTAAAGCTATTGTTTAATAATATTATTAAGGA 3519-20E3-R11 ATTAACTTAAATCTTTGATTGACTATATTTGAAT 3519-20E3-R12 AGGTTTTTGAATATATTAATCAAAACTATTGT 3519-20E3-R13 ATTTTGAATAAAAAAATTTCTTATTCCATGC 3519-20E3-R14 CAAAGAAAATCATCAGACAAAAAAGG 3519-20E3-R15 GAATTTGAATTTAACAATAAAAATTATTTATGCTT 3519-20E3-R16 GAATTTTTTGAAAAAATTTTTATTGCCAG 3519-20E3-R17 CTGTGAAAGAAAAATTTTTAAAAGTGAAAT 3519-20E3-R18 CAATATAGTGTTATTTTATGAGTTTAGGAAAG 3519-20E3-R19 TTTTGTTGGGGGATTTTTCAG 3519-20E3-R20 TTTTGTTGGGGGATTTTTCAG 3519-20E3-R21 GCAATATATTTATTTTTTTATTTATTTGTTTTATTGATATTA 3519-20E3-R22 GTATTATGATTGCTTTATTTGTTTATTACATTTC 3519-20E3-R23 GATATTATTTATCTTGTACTTATCTTTTTATGTTTT 3519-20E3-R24 GTCCCAAAATTGGAAAATTTTCC 3519-20E3-R25 TATTTAAAGAGCTTAAAATTAAGAGAAAAGATC BCT3511 gyrB 3511E3-F1 CGTGAAGCTGCAAGAAAA 3511E3-F2 TGGAAAAGCAATAAAAGCTGCTG 3511E3-F3 TGTTGTATATGAACATTTATTGGAAAT 3511E3-F4 GCTTGGTAATTCTGAGATAAGAAA 3511E3-F5 CCTCAATTTGAAGGTCAAACAAA 3511E3-F6 ATTTTAAAGAGGGGCTTACAGCT 3511E3-F7 GCCATGAATGAAGCTTTTAAA 3511E3-F8 CTCATGTTATGGGATTTAGAAGTGG 3511E3-F9 CTGACAACATTCTTCTTTTGTTAA 3511E3-F10 TGTTAATGTGGGGCTTAAATG 3511E3-F11 GCTTTTCAATCAGAACCTTATT 3511E3-F12 GAGGGTGGGATAAAATCTTTTT 3511E3-F13 TGGTAAAGAAAAATCTTCAAAATTTTAT 3511E3-F14 CGATAAAATATACATTTCAATTGAAGATAA 3511E3-F15 GGCTTAAAGAGCTTGCTTTT 3511E3-F16 AGATTATAATTTCGATGTTCTTGAAAAA 3511E3-F17 CGGATTCTGAAATTTTTGAAACTTT 3511E3-F18 GGGGACTAAGGTTACTTTTTT 3511E3-F19 AGAAGTTGTGGGGGAATCTTCTGTT 3511E3-F20 CTTTTTCAAAAGGTATTCCGACTT 3511E3-F21 GGTTTATGTTAATAGAGATGGAAAAAT 3511E3-F22 GGTTGTAAATGCTCTATCTTCGTT 3511E3-F23 TGGTAAGTTTAATAAAGGCACGTAT 3511E3-F24 CCTTGAACTTGTTTTAACAAAATTAC 3511E3-F25 ACCGATATTCATGAAGAGGAG 3511E3-R1 TACCCATTTTAGCACTTCCTCCA 3511E3-R2 TGGCAAAATGGCCTGAAAAA 3511E3-R3 TTGTTTTCTCAACATTAAGCATTTT 3511E3-R4 ATCATTGGTGATAACCTTATCTTCT 3511E3-R5 ACTCCTGCACCAAGAGAT 3511E3-R6 ATCTTGTGATAACGAAGTTTTGTA 3511E3-R7 TCCATCAACATCGGCATCTG 3511E3-R8 AAAAGCTAAAAGCAAAGTTCTAAT 3511E3-R9 ATATATCCATTTTCAATTAAATCTCTCAT 3511E3-R10 TATAAAGAGGAGGCATGGCT 3511E3-R11 TAAAAATAATAAATACGATTGTCATACTTT 3511E3-R12 TATTGCGATTTTTAGTTTCAATAGAA 3511E3-R13 CCCAAGCCCTTTATATCTCTGAA 3511E3-R14 AGCTGCGTTGGATTCATC 3511E3-R15 CTAGCAGGATCCATAGTTGTTT 3511E3-R16 ATCATCTATATTCATCAATCTCATTTTT 3511E3-R17 GAGTAACAAAAATTTTTTCAGCTTCA 3511E3-R18 TTTCTGGGCTCAACTAAATCT 3511E3-R19 GATTAATTACATTAAGTGCATTCTGTTC 3511E3-R20 CCATTAACGCTCCAATTACAC 3511E3-R21 TCCTAACATTTAATATTTGTTCTTTATTTTC 3511E3-R22 GCATAATTTAAATAAGAAGTTTTTATTTCATCT 3511E3-R23 GAAGAGCTCTAGAAACAATAACTGA 3511E3-R24 TGGTTTAAGACCATCTCTTACGT 3511E3-R25 CTCATACATAGAATAAAGTATTCTCCTG

Since two of the target regions are close a single set of flanking oligos was designed to cover both targets. All primers were brought up to an initial concentration of 1 mM in 10 mM Tris pH 8.0 and 50 uM EDTA (pH 8.0). The primers were mixed in equal proportions to create a 1 mM oligo mix. Primers were designed using B. burgdorferi B31 genome sequence (gi|15594346) and have a GC content of 25 to 50%, spaced 6-10 nucleotides apart and have a target TM of 52° C. To ensure removal of any contaminating salts the pooled primers were dialyzed twice for 4 hours at 4° C. against a 4 L solution containing 10 mM Tris pH 8.0 and 50 uM EDTA pH 8.0 using a 5 mL Float-A-Lyzer G2 (Spectrum Laboratories, Rancho Dominguez, Calif.) with a molecular weight cutoff of 0.5-1 kDa.

The nested isothermal amplification was performed in a 225 ul reaction in a 0.6 mL PCR tube (Axygen Inc., Union City, Calif.) containing 200 uL of nucleic acid extract, 22.5 ul Ibis 10× PCR Buffer II²¹ (Ibis Biosciences, Carlsbad, Calif.), 0.2 uM dNTPs (Bioline, Tauton, Mass.), and 10 uM oligo mix. The reactions were incubated at 95° C. for 10 min followed by a cooling to 56° C. in a MJ Thermocycler (Bio-Rad Laboratories, Hercules, Calif.). The reactions were then removed to a heat block at 56° C. and 11.25 U of BstE DNA polymerase (Lucigen, Middleton, Wis.) enzyme added and the reactions incubated at 56° C. for 2 hours followed by an 80° C. heat inactivation for 20 min. The resulting reaction was used directly in the subsequent PCR without purification.

Detection of B. burgdorferi from Whole Blood from Patients with Clinically Diagnosed Early Lyme Disease.

Borrelia was detected by processing 2 ul of Borrelia enriched nucleic acid extracts per PCR reaction on a previously described broad-range PCR/ESI-MS assay designed to detect and characterize Borrelia burgdorferi as previously described.²¹. Electrospray ionization mass spectrometry was performed on the PLEX-ID biosensor (Abbott Molecular). Briefly, after PCR amplification, 30 μL aliquots of each PCR reaction were desalted and analyzed by mass spectrometry as previously described²¹⁻²³ (herein incorporated by reference as if fully set forth herein). Analysis of amplicons from any one of the eight primer pairs in the assay can be used to positively identify Borrelia DNA in a specimen.

Results

The data are supportive that this new strategy can positively impact current clinical and laboratory impediments to early diagnosis of Lyme disease. A serendipitous finding of clinical importance was that the majority (˜60%), of rashes were not the classic EM in PCR positive cases.

Detection of Lyme disease in 29 patients with classic and non-classic EM Examination of nucleic acid extract from 1.25 ml of whole blood from the independent set of 29 endemic patients with clinically diagnosed Lyme disease with classic or non-classic EM and 44 healthy controls showed that 14 of the 29 Lyme patients, and 0 of 45 controls, (48%, p=0.0001) had detectable B. burgdorferi. The pre-PCR enrichment step enabled increased detection of Borrelia from 2 to 14 cases (7×) when assessed by the PCR/ESI-MS assay. Two-tiered serology was positive in 14 of the 29 specimens, not all of which overlapped with the 14 specimens positive by NIA/PCR/ESI-MS from Table 2. Nine of the clinically defined early Lyme disease specimens tested negative by both PCR and serology assays. However, we did not have skin isolates to determine if the Borrelia was actually present as a skin-restricted strain which did not disseminate to blood.^(23,24) Table 2 is presented to show PCR detection is possible even when serology is negative or not yet positive. The data support the concept that unambiguous diagnosis can be made early, before seroconversion.

TABLE 2 EM, B. burgdorferi PCR and serological analysis of 14 Early Lyme disease specimens positive by NIA/PCR/ESI-MS from whole blood. PCR Early 2-tier Follow-up two-tier EM PCR # IgM # IgG # IgM # IgG ID EM¹ Result Result² ELISA bands bands Result² ELISA bands bands 26 NC Pos Neg ≦0.90 — — Pos  4.35 3 1 33 C Pos Pos >5.00 3 4 ND — — — 37 C Pos Neg 1 1 3 Pos >5.00 3 5 40 NC Pos Pos >5.00 3 4 ND — — — 44 NC Pos Neg ≦0.90 — — Pos >5.00 3 6 45 NC Pos Neg 1.36 1 1 Pos >5.00 2 2 46 NC Pos Pos >5.00 3 1 ND — — — 47 C Pos Pos >5.00 3 4 ND — — — 48 NC Pos Neg ≦0.90 — — Neg  1.46 1 2 49 NC Pos Pos 2.49 2 0 ND — — — 51 C Pos Neg 4.49 1 3 Neg >5.00 2 4 52 NC Pos Pos 3.54 2 3 ND — — — 53 NC Pos Pos 4.73 3 2 ND — — — 54 NC Pos Pos 2.86 2 2 ND — — — ¹C = classic erythema migrans; NC= non-classic erythema migrans ²Positivity based upon CDC two tiered serologic criteria Results illustrated for 14/29 patients who were PCR+. Pos = positive, Neg = negative, ND = not done Of the 14 early Lyme specimens that tested positive by the NIA/PCR/ESI-MS assay, 6 were negative by the 2-tiered test at the time of presentation before the initiation of antibiotics (Table 2). Of these 6 specimens, 4 seroconverted by the follow-up serological testing 3 weeks later indicating that these were likely recent infections. Two of the NIA/PCR/ESI-MS positive specimens (#48 and #51) did not seroconvert sufficiently to meet the CDC surveillance criteria²⁵ but both specimens showed an increase in ELISA titers and increased IgG/IgM blot reactivity, indicating that these patients were most likely represent weak or slow responders possibly due to antibiotic therapy²⁶ or for unknown reasons. Of the 44 control patient sera, a single sample was seropositive by ELISA and IgG western blot, but was PCR negative. This low rate in our sample set from the eastern United States is consistent with the known background seroreactivity from remote exposure in an endemic region.

These results demonstrate that B. burgdorferi infection can be diagnosed early, and even prior to seroconversion, from whole blood in a high percentage of patients with suspected Lyme using a pre-PCR Borrelia-DNA enhancing method coupled with PCR/ESI-MS assay. Other isothermal amplification methods to generate genetic material has been described but not for Borrelia. ^(7,8) In this case, a novel nested isothermal amplification (NIA) was coupled with a PCR/ESI-MS assay and results were contrasted with the two-tier serology. However, in a clinical situation, finding Borrelia DNA circulating in blood in an ill person with endemic area exposure will have such a strong possibility of a current infection that it would support a clinical decision to treat regardless of whether there is a classical EM, an atypical skin lesion, or extracutaneous systemic symptoms and signs suggestive of Lyme disease. The could allow for early diagnosis of the 20-30% of patients with early Lyme disease that present with “viral-like” symptoms indistinguishable for other community acquired infectious diseases. In contrast, a single serologic test, even if positive, may be difficult to interpret in a person living in an endemic area because this single result could represent past exposure. The present strategy has the potential to remove this ambiguity.

Work conducted during development of embodiments of the present invention led to the conclusion that hold blood may be preferable to serum or plasma for detection of Borrelia. While not limited to any mechanism, this may be due to the pathogen adhering to particular blood cells. In contrast to many diagnostics based on analysis of small (ul) of samples, the present disclosure is configured to handle larger volumes (mls), but within clinical practice volumes, to increase the detection of pathogens that may be present only in low copy numbers. A recent paper²⁷ showed that B. burgdorferi may be present in a high percentage of patients with Lyme disease but may require “teasing” it out with combinations of cultures and PCR. Although this method is not as easily performed within a clinically useful time period, as that which is described herein, it does suggest that there is an attainable target should it be present.

A serendipitous observation in this Example and an important clinical finding was the high percentage (57%) of PCR positive patients whose skin rash was not the classical EM but an atypical lesion (see FIG. 1) that could be easily misdiagnosed. Photographs of lesions (all greater than 5 cm) were presented to four physicians experienced with Lyme disease, including two dermatologists. Without knowledge of the laboratory data they were asked to categorize the lesions into 1) those that they would expect any reasonably trained physician to recognize as EM and 2) into those that they would not fault such a physician from referring the patient or desiring supportive laboratory tests or more time for observation.^(28,29) Based on previous reports, including a vaccine trial, of atypical rashes in 25-30% of microbiologically confirmed B. burgdorferi infected subjects^(4,5) it was expected a similar percentage, but were surprised by almost 60%. This high percentage serves as an alert for physicians to consider Lyme disease in the differential diagnosis of patients with endemic area exposure and a rash that is not the classic EM. These atypical lesions serve as a reminder of the need for diagnostics for the endemic area patient who only has a flu-like illness during the high season for Lyme disease. Such a patient may benefit from the testing strategy described in this Example or, at the very least, closer monitoring.

It is believed that these results demonstrate a useful strategy to the diagnosis of infections when there is a paucity of pathogens or the immune response cannot provide an unambiguous result. It is likely that many of these difficult to diagnose infections will require a battery of diagnostic platforms each with advantages depending on when the patient presents.

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All publications and patents mentioned in the present application are herein incorporated by reference. Various modification and variation of the described methods and compositions of the invention will be apparent to those skilled in the art without departing from the scope and spirit of the invention. Although the invention has been described in connection with specific preferred embodiments, it should be understood that the invention as claimed should not be unduly limited to such specific embodiments. Indeed, various modifications of the described modes for carrying out the invention that are obvious to those skilled in the relevant fields are intended to be within the scope of the following claims. 

We claim:
 1. A method of nucleic acid extraction comprising: a) contacting a sample whole blood with beads, a proteinase, and an anionic surfactant to generate a treated sample; b) homogenizing said treated sample to generate a cell lysate; c) centrifuging said cell lysate comprising a supernatant; d) separating said supernatant from said cell lysate; e) adding magnetic particles and lysis buffer to said supernatant to generate a magnetic-particle sample, wherein said magnetic particles are configured to bind nucleic acid molecules; f) washing said magnetic-particle sample with a wash buffer; g) treating said magnetic-particle sample in order to generate a dried magnetic bead sample; and h) treating said dried magnetic bead sample with an elution buffer such that a purified nucleic acid sample is generated that comprises purified nucleic acid.
 2. The method of claim 1, further comprising subjecting said purified nucleic acid to PCR and/or isothermal nested PCR to generate amplified nucleic acid.
 3. The method of claim 2, further subjecting said amplified nucleic acid to mass spectrometry bioagent analysis in order to identify the source of said purified nucleic acid.
 4. The method of claim 3, wherein said mass spectrometry bioagent analysis comprises electrospray ionization mass spectrometry and base composition analysis.
 5. A method comprising: a) contacting a sample comprising isolated nucleic acid with a buffer, dNTPs, and a plurality of nested PCR primer pairs configured to amplify at least part of at least one bioagent target sequence; b) incubating said sample with a DNA polymerase under isothermal conditions such that amplified nucleic acid is generated; c) inactivating said DNA polymerase; and d) subjecting said amplified nucleic acid to mass spectrometry bioagent analysis in order to identify the source of said isolated nucleic acid.
 6. The method of claim 5, wherein said mass spectrometry bioagent analysis comprises electrospray ionization mass spectrometry and base composition analysis.
 7. The method of claim 5, wherein said DNA polymerase comprises BstE DNA polymerase.
 8. The method of claim 5, wherein said incubating is conducted at about 56 degrees Celsius.
 9. The method of claim 5, wherein said inactivating said DNA polymerase comprises heating said sample to at least about 80 degrees Celsius.
 10. The method of claim 5, wherein said plurality of nested PCR primer pairs comprises at least 10 primer pairs.
 11. The method of claim 5, wherein said plurality of nested PCR primer pairs comprises at least 20 primer pairs.
 12. The method of claim 5, wherein said at least one bioagent target sequence comprises at least five bioagent target sequences.
 13. The method of claim 5, further comprising a step after c) but before d) of further amplifying said amplified nucleic acid without any purification of said amplified nucleic acid. 